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采用短串联重复序列位点多重扩增的自动化DNA分型

Automated DNA profiling employing multiplex amplification of short tandem repeat loci.

作者信息

Kimpton C P, Gill P, Walton A, Urquhart A, Millican E S, Adams M

机构信息

Central Research and Support Establishment, Forensic Science Service, Reading, Berks, United Kingdom.

出版信息

PCR Methods Appl. 1993 Aug;3(1):13-22. doi: 10.1101/gr.3.1.13.

Abstract

We have employed automated fluorescence-based technology to detect amplified tri-, tetra-, and pentanucleotide short tandem repeat (STR) loci electrophoresed on denaturing polyacrylamide sequencing gels. The system described incorporates an internal size standard in each sample, allowing the STR-PCR products to be sized automatically with a high degree of precision. By utilizing different fluorescent dye markers for loci that have overlapping allele size ranges, we have developed three multiplex STR systems containing a total of 14 different loci. These multiplex systems were then used to evaluate the usefulness of the 14 loci for the identification of individuals. Allele frequency data were collected from a minimum of 50 individuals from each of three different racial groups: Caucasians, Afro-Caribbeans, and Asians. Of the resulting 42 locus population sets, deviation from Hardy-Weinberg equilibria was detected in only the STR HUMCYARO3-Caucasian data. The probabilities of two unrelated individuals matching by chance (pM) at all 14 loci in the three multiplex reactions was < 1 x 10(14). The combination of multiplex STR-PCR and automatic fluorescence-based detection is thus a rapid and powerful technique for individual identification.

摘要

我们采用了基于荧光的自动化技术,以检测在变性聚丙烯酰胺测序凝胶上电泳的三核苷酸、四核苷酸和五核苷酸短串联重复序列(STR)位点的扩增情况。所描述的系统在每个样本中加入了内部大小标准,从而能够高精度地自动测定STR-PCR产物的大小。通过对具有重叠等位基因大小范围的位点使用不同的荧光染料标记,我们开发了三个多重STR系统,总共包含14个不同的位点。然后使用这些多重系统来评估这14个位点在个体识别中的实用性。等位基因频率数据是从三个不同种族群体(白种人、非裔加勒比人和亚洲人)中至少50个个体收集的。在所得的42个位点群体数据集中,仅在STR HUMCYARO3 - 白种人数据中检测到偏离哈迪-温伯格平衡的情况。在三个多重反应中,两个无关个体在所有14个位点偶然匹配的概率(pM)<1×10⁻¹⁴ 。因此,多重STR-PCR与基于荧光的自动检测相结合是一种快速且强大的个体识别技术。

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